Maribavir isomers, compositions, methods of making and methods of using

ABSTRACT

The invention relates to novel compositions and methods of using maribavir which enhance its effectiveness in medical therapy, as well as to maribavir isomers and methods of use thereof for counteracting the potentially adverse effects of maribavir isomerization in vivo in the event it occurs.

CROSS-REFERENCE TO RELATED APPLICATIONS

The present application is a divisional of U.S. patent application Ser. No. 15/055,043, filed Feb. 26, 2016, which is a continuation of U.S. patent application Ser. No. 14/595,548, filed Jan. 13, 2015, which is a continuation of U.S. Pat. No. 8,940,707, filed Oct. 27, 2011, which claims the benefit of U.S. Provisional Patent Application No. 61/407,637, filed Oct. 28, 2010, the entire disclosure of which is incorporated by reference herein.

BACKGROUND OF THE INVENTION

The present invention relates to compositions and methods for enhancing the therapeutic efficacy of the compound 5,6-dichloro-2-(isopropylamino)-1-(β-L-ribofuranosyl)-1H-benzimidazole (also known as 1263W94 and maribavir), as well as to maribavir isomers and a method of making such isomers.

5,6-dichloro-2-(isopropylamino)-1-(β-L-ribofuranosyl)-1H-benzimidazole is a benzimidazole derivative useful in medical therapy. U.S. Pat. No. 6,077,832 discloses 5,6-dichloro-2-(isopropylamino)-1-(β-L-ribofuranosyl)-1H-benzimidazole and its use for the treatment or prophylaxis of viral infections such as those caused by herpes viruses. The compound as disclosed in U.S. Pat. No. 6,077,832 is an amorphous, non-crystalline material.

The structure of 5,6-dichloro-2-(isopropylamino)-1-(β-L-ribofuranosyl)-1H-benzimidazole is:

The preparation of certain unique crystalline forms and solvate forms of maribavir, as well as pharmaceutical formulations thereof and their use in therapy are described in U.S. Pat. Nos. 6,469,160 and 6,482,939.

The present invention has arisen out of the unexpected discovery that maribavir may isomerize under in vivo conditions to one or more configurational stereoisomers or constitutional isomers. The maribavir compound contains 4 (four) chiral carbon centers in the ribofuranosyl moiety and therefore maribavir is just one of 16 (sixteen) potential stereoisomers that may be formed under various in vivo conditions.

Under in vivo conditions, maribavir can isomerize to other compounds that may (or may not) have the same or similar chemical, physical and biological properties. The in vivo isomerization of maribavir results in conversion of maribavir to other isomers that have the same molecular formula but a different molecular structure. The different molecular structures can be grouped into isomers that have different connectivity of the constituent atoms (constitutional isomers) or grouped into isomers that have the same “connectivity” but differ in the way the atoms and groups of atoms are oriented in space (configurational stereoisomers). Such molecular conversion in vivo is believed to result in the dilution of the effective maribavir concentration in the host that was treated with maribavir. The in vivo isomerization transforms and distributes dosed maribavir material into other molecular entities that do not necessarily have the same or similar biological activity. If the isomerization results in the formation of isomers that have a lower degree of corresponding biological activity relative to the activity of maribavir, then the isomerization will decrease the effective biological activity of maribavir dose administered to a host.

A recent maribavir Phase 3 clinical trial conducted by ViroPharma Incorporated (the 300 Study) that evaluated maribavir for cytomegalovirus (CMV) prophylaxis in allogeneic stem cell, or bone marrow, transplant (SCT) patients did not achieve its primary endpoint. In the primary analysis, there was no statistically significant difference between maribavir and placebo in reducing the rate of CMV disease. In addition, the study failed to meet its key secondary endpoints (ViroPharma Press Release dated Feb. 9, 2009). The 300 Study result appeared at first blush to be inconsistent with an earlier proof-of-concept (POC) maribavir Phase 2 clinical trial (the 200 Study) wherein ViroPharma reported positive preliminary results that showed that maribavir inhibited CMV reactivation in SCT patients. The data from this study demonstrate that prophylaxis with maribavir displays strong antiviral activity, as measured by significant reduction in the rate of reactivation of CMV in recipients of allogeneic stem cell (bone marrow) transplants, and that administration of maribavir for up to 12 weeks has a favorable tolerability profile in this very sick patient population (ViroPharma Press Release date Mar. 29, 2006).

However, the 300 Study result can be explained in terms of the instant maribavir isomerization theory/discovery. An unrecognized key difference between the 200 Study and the 300 Study was that the former provided for a fasted dosing protocol of maribavir, whereas the latter allowed the dosing protocol to be either under fasted or fed conditions (at the discretion of the clinician). The nature of the patient population in the 300 Study suggests that probably very few patients were dosed under the strict fasted dosing protocol that was previously used in the 200 Study. The change in dosing protocol in the 300 Study changed not only the in vivo dosing conditions for maribavir, but also the nature and/or degree of isomerization of maribavir that occurs in vivo, so that more maribavir was isomerized to other less effective compounds, thereby reducing the effective bioavailable concentration of maribavir drug below levels necessary to adequately prevent CMV infection and/or CMV re-activation in the host.

The degree and nature of the isomerization of maribavir depends on the particular in vivo conditions to which the drug is exposed, which are variable. The potential mechanisms for isomerizing maribavir in vivo are by chemical isomerization (acid, base and/or metal catalyzed isomerization), microbially-mediated isomerization, and/or host metabolism induced isomerization. See, for example, Okano, Kazuya, Tetrahedron, 65: 1937-1949 (2009); Kelly, James A. et al., J. Med. Chem., 29: 2351-2358 (1986); and Ahmed, Zakaria et al., Bangladesh J. Sci. Ind. Res., 25(1-4): 90-104 (2000).

Thus, maribavir should be formulated, administered, packaged and promoted in ways that will prevent or at least reduce the unwanted occurrence of maribavir isomerization in vivo, thereby enhancing the drug's bioavailability and efficacy, and/or counteract the potential adverse effect(s) of maribavir isomerization in vivo, if it occurs.

SUMMARY OF THE INVENTION

The invention generally relates to the unexpected discovery that maribavir may isomerize under in vivo conditions to one or more configurational stereoisomers and/or constitutional isomers. Aspect of the invention is illustrated below.

The practical applications of the instant discovery and related inventions are as follows:

-   -   (1) The invention includes methods of making maribavir isomers         under in vivo conditions (method of administering maribavir as a         prodrug to make other maribavir isomers).     -   (2) The invention includes methods dosing maribavir so as to         mitigate the impact of in vivo maribavir isomerization (such as         dosing under fasted conditions, or increasing the dose of         maribavir).     -   (3) The invention includes maribavir formulations that         effectively mitigate the adverse effects of in vivo maribavir         isomerization (quick release formulations, delayed/controlled         release formulations, combination with antacids,         intravenous (IV) formulations, combination formulations with         antibiotics to prevent microbial isomerization).     -   (4) The invention includes methods of using one or more         maribavir isomers to prevent or treat disease in host (as         antivirals, for example for treating/preventing CMV, EBV, HCV).     -   (5) The invention includes methods of using one or more         maribavir isomers as reference standards in analytical methods         for monitoring the blood plasma concentrations of maribavir and         related isomers.     -   (6) The invention includes methods of monitoring maribavir and         maribavir isomers, and using the information to adjust treatment         protocols (increase/decrease dose, change dosing regimen         fed/fasted, discontinue maribavir therapy, start other therapy).         The analytical methods for monitoring in vivo maribavir         concentrations must be able discriminate between maribavir and         maribavir isomers (for example chiral chromatography, and in         particular LC-MS-MS using a chiral sorbent material in the LC         column).     -   (7) The invention includes a method of more safely and         effectively using maribavir to treat or prevent disease in         humans by including information and guidance in the product         label and/or promotional materials to inform the public as to         how to use the maribavir product so as to avoid or to mitigate         the adverse impact of in vivo maribavir isomerization, and thus         optimize therapeutic efficacy and safety.     -   (8) The invention includes the corresponding inventions related         to the maribavir isomers that are pyranosyl constitutional         isomers of maribavir.

The present invention also relates to a package or kit comprising therapeutically effective dosage forms of maribavir, prescribing information and a container for the dosage form. The prescribing information includes advice to a patient receiving maribavir therapy regarding the administration of maribavir without food to improve bioavailability.

DETAILED DESCRIPTION OF THE INVENTION

The following table contains list of useful dosing protocols that may be used to improve the efficacy and safety for treating a patient with maribavir.

Fasting Maribavir conditions Route of admin- dosing Dosing (before/after istration and Protocol amount dosing) dosage form. 01 3200 mg/ None Oral - tablet - 2 x day immediate release 02 3200 mg/ None IV 2 x day 03 1600 mg/ None Oral - tablet - 2 x day w/antacids 04 1600 mg/ None Oral- tablet - 1 x day w/antibiotics 05 800 mg/ None Oral- tablet - 3 x day delayed release 06 800 mg/ None Oral- tablet - 2 x day immediate release 07 800 mg/ None IV 1 x day 08 400 mg/ None Oral - tablet - 4 x day w/antacids 09 400 mg/ None Oral- tablet - 3 x day w/antibiotics 10 400 mg/ None Oral- tablet - 2 x day delayed release 11 400 mg/ None Oral - tablet - 1 x day immediate release 12 3200 mg/ 12 hrs/ IV 2 x day 3 hrs 13 3200 mg/ 12 hrs/ Oral - tablet - 2 x day 3 hrs w/antacids 14 1600 mg/ 12 hrs/ Oral- tablet - 2 x day 3 hrs w/antibiotics 15 1600 mg/ 12 hrs/ Oral- tablet - 1 x day 3 hrs delayed release 16 800 mg/ 12 hrs/ Oral- tablet - 3 x day 3 hrs immediate release 17 800 mg/ 12 hrs/ IV 2 x day 3 hrs 18 800 mg/ 12 hrs/ Oral - tablet - 1 x day 3 hrs w/antacids 19 400 mg/ 12 hrs/ Oral- tablet - 4 x day 3 hrs w/antibiotics 20 400 mg/ 12 hrs/ Oral- tablet - 3 x day 3 hrs delayed release 21 400 mg/ 12 hrs/ Oral - tablet - 2 x day 3 hrs immediate release 22 400 mg/ 12 hrs/ Oral- tablet - 1 x day 3 hrs immediate release 23 3200 mg/ 6 hrs/ Oral - tablet - 2 x day 2 hrs immediate release 24 3200 mg/ 6 hrs/ IV 2 x day 2 hrs 25 1600 mg/ 6 hrs/ Oral - tablet - 2 x day 2 hrs w/antacids 26 1600 mg/ 6 hrs/ Oral- tablet - 1 x day 2 hrs w/antibiotics 27 800 mg/ 6 hrs/ Oral- tablet - 3 x day 2 hrs delayed release 28 800 mg/ 6 hrs/ Oral- tablet - 2 x day 2 hrs immediate release 29 800 mg/ 6 hrs/ IV 1 x day 2 hrs 30 400 mg/ 6 hrs/ Oral - tablet - 4 x day 2 hrs w/antacids 31 400 mg/ 6 hrs/ Oral- tablet - 3 x day 2 hrs w/antibiotics 32 400 mg/ 6 hrs/ Oral- tablet - 2 x day 2 hrs delayed release 33 400 mg/ 6 hrs/ Oral - tablet - 1 x day 2 hrs immediate release 34 3200 mg/ 3 hrs/ IV 2 x day 1 hr 35 3200 mg/ 3 hrs/ Oral - tablet - 2 x day 1 hr w/antacids 36 1600 mg/ 3 hrs/ Oral- tablet - 2 x day 1 hr w/antibiotics 37 1600 mg/ 3 hrs/ Oral- tablet - 1 x day 1 hr delayed release 38 800 mg/ 3 hrs/ Oral- tablet - 3 x day 1 hr immediate release 39 800 mg/ 3 hrs/ IV 2 x day 1 hr 40 800 mg/ 3 hrs/ Oral - tablet - 1 x day 1 hr w/antacids 41 400 mg/ 3 hrs/ Oral- tablet - 4 x day 1 hr w/antibiotics 42 400 mg/ 3 hrs/ Oral- tablet - 3 x day 1 hr delayed release 43 400 mg/ 3 hrs/ Oral - tablet - 2 x day 1 hr immediate release 44 400 mg/ 3 hrs/ Oral- tablet - 1 x day 1 hr immediate release

In carrying out the method of the invention, it is preferably to determine the presence and/or concentration of maribavir isomers, especially isomers of diminished therapeutic efficacy in patient blood plasma samples as part of the method.

As used herein, the terms “fasted conditions”, “fasting conditions” and “without food” are defined to mean, in general, the condition of not having consumed food during the period between from at least about 3 to 12 hours prior to the administration of maribavir to at least about 1 to 3 hours after the administration of maribavir. Other narrower “fasted conditions” are also contemplated herein and described below.

The term “with food” is defined to mean, in general, the condition of having consumed food prior to, during and/or after the administration of maribavir that is consistent with the relevant intended definition of “fasted conditions” (which may be narrow or broad depending on the circumstances). Preferably, the food is a solid food sufficient bulk and fat content that it is not rapidly dissolved and absorbed in the stomach. More preferably, the food is a meal, such as breakfast, lunch or dinner.

The term “isomers” means compounds that have the same molecular formula but a different molecular structure.

The term “constitutional isomers” is defined to mean isomers that have the same molecular formula but a different molecular structure wherein the molecular structures of the isomers have different connectivity of the constituent atoms.

The term “configurational stereoisomers” is defined to mean isomers that have the same “connectivity” but differ in the molecular structure in the way the atoms and groups of atoms are oriented in space.

The term “immediate release” is defined to mean release of drug from drug formulation by dissolution is less than 60 minutes or is otherwise release from the drug formulation in less than 60 minutes.

The term “IV” is defined to mean intravenous.

The chemical structure of maribavir and some maribavir isomers are shown below. The instant invention contemplates novel formulations, dosage levels and methods of use of maribavir, the maribavir isomers MFI-01 to MFI-015 (configurational stereoisomers), as well as the maribavir isomers MPI-01 to MPI-016 (constitutional isomers). The invention also contemplates the corresponding acyclic constitutional isomers wherein the sugar moiety is an open chain and attached to the benzimidazole.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 shows chemical structures of maribavir and maribavir configurational stereoisomers that have the same configuration at the furanosyl anomer carbon.

FIG. 2 shows chemical structures of maribavir configurational stereoisomers that have the opposite configuration at the furanosyl anomer carbon.

FIG. 3 shows chemical structures of maribavir “pyranosyl” constitutional isomers)

A number of patent and non-patent documents are cited in the foregoing specification in order to describe the state of the art to which this invention pertains. The entire disclosure of each of these citations is incorporated by reference herein.

While certain of the preferred embodiments of the present invention have been described and specifically exemplified above, it is not intended that the invention be limited to such embodiments. Various modifications may be made thereto without departing from the scope and spirit of the present invention, as set forth in the following claims. Furthermore, the transitional terms “comprising”, “consisting essentially of” and “consisting of” define the scope of the appended claims, in original and amended form, with respect to what unrecited additional claim elements or steps, if any, are excluded from the scope of the claims. The term “comprising” is intended to be inclusive or open-ended and does not exclude additional, =recited elements, methods step or materials. The phrase “consisting of” excludes any element, step or material other than those specified in the claim, and, in the latter instance, impurities ordinarily associated with the specified materials. The phrase “consisting essentially of” limits the scope of a claim to the specified elements, steps or materials and those that do not materially affect the basic and novel characteristic(s) of the claimed invention. All compositions or formulations identified herein can, in alternate embodiments, be more specifically defined by any of the transitional phases “comprising”, “consisting essentially of” and “consisting of”. 

What is claimed is:
 1. A method for treatment of a herpes viral infection in a patient in need thereof comprising administering to the patient an amount of the compound 5,6-dichloro-2-(isopropylamino)-1-(β-L-ribofuranosyl)-1H-benzimidazole, wherein the patient is receiving or has received at least one of: i) an antacid which is effective for neutralizing acid that catalyzes isomerization of the compound, ii) an antibiotic having activity against a microorganism that mediates isomerization of the compound, or iii) an antagonist that inhibits metabolism that induces isomerization of the compound; thereby providing an anti-virally effective amount of the compound to the patient.
 2. A method of claim 1, wherein the amount of the compound administered is greater than 200 mg per day.
 3. A method of claim 2, wherein the amount of the compound administered is up to 6400 mg per day.
 4. A method of claim 1, wherein the herpes viral infection is cytomegalovirus.
 5. A method of claim 4, wherein the patient is a stem cell transplant recipient, a liver transplant recipient, or kidney transplant recipient.
 6. A method of claim 1, wherein the compound is administered to the patient under fasted conditions.
 7. The method of claim 1, wherein the compound is administered as a composition comprising a therapeutically acceptable adjuvant, excipient or carrier medium.
 8. The method of claim 7, wherein the composition is an immediate release formulation, a delayed release formulation, a controlled release formulation or an intravenous formulation.
 9. The method of claim 1, wherein the isomerization of the compound would decrease the therapeutic efficacy of the compound. 